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Nov 29, 2007 - coronavirus and InfA H5N1 in a multiplex assay would allow ...... PCR assays for absolute quantitation of human coronaviruses OC43 and.
JOURNAL OF CLINICAL MICROBIOLOGY, Apr. 2008, p. 1232–1240 0095-1137/08/$08.00⫹0 doi:10.1128/JCM.02294-07 Copyright © 2008, American Society for Microbiology. All Rights Reserved.

Vol. 46, No. 4

RespiFinder: a New Multiparameter Test To Differentially Identify Fifteen Respiratory Viruses䌤 Martin Reijans,1* Gijs Dingemans,1† Corne´ H. Klaassen,1 Jacques F. Meis,1 Judith Keijdener,2 Brit Mulders,2 Kimberly Eadie,3 Willem van Leeuwen,3 Alex van Belkum,3 Alphons M. Horrevorts,1 and Guus Simons2 Department of Medical Microbiology and Infectious Diseases, Canisius Wilhelmina Hospital, Nijmegen, The Netherlands1; PathoFinder BV, Maastricht, The Netherlands2; and Department of Medical Microbiology and Infectious Diseases, Erasmus Medical Center Rotterdam, Rotterdam, The Netherlands3 Received 29 November 2007/Returned for modification 2 January 2008/Accepted 25 January 2008

Broad-spectrum analysis for pathogens in patients with respiratory tract infections is becoming more relevant as the number of potential infectious agents is still increasing. Here we describe the new multiparameter RespiFinder assay, which is based on the multiplex ligation-dependent probe amplification (MLPA) technology. This assay detects 15 respiratory viruses in one reaction. The MLPA reaction is preceded by a preamplification step which ensures the detection of both RNA and DNA viruses with the same specificity and sensitivity as individual monoplex real-time reverse transcription-PCRs. The RespiFinder assay was validated with 144 clinical samples, and the results of the assay were compared to those of cell culture and a respiratory syncytial virus (RSV)-specific immunochromatography assay (ICA). Compared to the cell culture results, the RespiFinder assay showed specificities and sensitivities of 98.2% and 100%, respectively, for adenovirus; 96.4% and 100%, respectively, for human metapneumovirus; 98.2% and 100%, respectively, for influenza A virus (InfA); 99.1% and 100%, respectively, for parainfluenza virus type 1 (PIV-1); 99.1% and 80%, respectively, for PIV-3; 90.1% and 100%, respectively, for rhinovirus; and 94.6% and 100%, respectively, for RSV. Compared to the results of the RSV-specific ICA, the RespiFinder assay gave a specificity and a sensitivity of 82.4% and 80%, respectively. PIV-2, PIV-4, influenza B virus, InfA H5N1, and coronavirus 229E were not detected in the clinical specimens tested. The use of the RespiFinder assay resulted in an increase in the diagnostic yield compared to that obtained by cell culture (diagnostic yields, 60% and 35.5%, respectively). In conclusion, the RespiFinder assay provides a user-friendly and high-throughput tool for the simultaneous detection of 15 respiratory viruses with excellent overall performance statistics. rapid diagnosis could be helpful in therapeutic decision making. In addition, there is an increasing threat of uncommon yet significant respiratory viruses, such as the severe acute respiratory syndrome (SARS) coronavirus and influenza A virus (InfA) H5N1 (28). As a result, it is becoming more important to detect a broad panel of respiratory viruses. Cell culture is still the “gold standard” for the laboratory detection of respiratory viruses. However, cell culture is slow and has a low sensitivity. Therefore, its implementation for routine virus detection is suboptimal. Although rapid antigen detection tests are available for some of the respiratory viruses, these tests have been shown to be less sensitive and less specific than cell culture-based approaches (5, 29). Nucleic acid amplification tests have proven to be rapid, very sensitive, and specific alternatives and can be used in either a monoplex or a multiplex format. Moreover, multiplex assays allow the coamplification of more than one target, thus providing insight into the significance of mixed infections for the prognosis and recrudescence of the respiratory disease. In addition, the incorporation of the ability to detect viruses such as the SARS coronavirus and InfA H5N1 in a multiplex assay would allow monitoring of these viruses and could act as an early built-in detection system (28). An all-embracing multiparameter test is a prerequisite to reducing the costs involved with such a comprehensive monitoring system (19). Currently, several assays with multiplex formats detect up to nine respiratory viruses in one reaction.

Acute respiratory tract infections (RTIs) are the most widespread types of infections in adults and children and are responsible for considerable morbidity and mortality worldwide (18). Unfortunately, the etiology remains undetermined in more than 50% of cases (9). Among the pathogens responsible for undiagnosed infections, respiratory viruses are thought to contribute to a substantial number of RTIs. Influenza viruses, respiratory syncytial viruses (RSVs), and parainfluenza viruses (PIVs) have been identified as important pathogens in community-acquired pneumoniae. These viruses are also a significant cause of disease in immunocompromised patients (11). Currently, the clinical diagnosis of RTIs is mostly restricted to the detection and identification of these few pathogens. However, evidence is accumulating that other viruses, such as coronaviruses 229E, OC43, and NL63 (Cor-OC43, Cor-229E, and Cor-NL63, respectively) (35) and human metapneumovirus (hMPV) (20, 33), are frequently associated with infected lower respiratory tracts. Even an unexpectedly high prevalence of rhinovirus in lower RTIs has been demonstrated in children as well as adults (8). The clinical presentation of patients with RTIs is generally not indicative of a specific pathogen, so a

* Corresponding author. Present address: PathoFinder B.V., Oxfordlaan 70, 6229 EV Maastricht, The Netherlands. Phone: 31(0)433885852. Fax: 31(0)847469245. E-mail: [email protected]. † Present address: PathoFinder B.V., Maastricht, The Netherlands. 䌤 Published ahead of print on 6 February 2008. 1232

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For instance, several real-time multiplex assays allow the realtime detection of up to four targets in a reaction, depending on the number of channels available in the real-time PCR machines (13, 30, 34). Based on the Roche LightCycler480 instrument, a real-time TaqMan PCR that detects five different targets simultaneously has been developed (21). Existing multiplex PCR assays that use agarose gel electrophoresis or capillary electrophoresis as the detection system detect five to eight targets per reaction (3, 7, 24). Multiplex PCR assays combined with an enzyme-linked immunosorbent assay currently detect up to nine targets simultaneously (12, 26). Recently, two multiplex assays that detect respiratory viruses have been evaluated with 360 clinical samples (17). The NGEN respiratory virus analyte-specific assay (Nanogen, San Diego, CA) detects InfA, InfB, PIV type 1 (PIV-1), PIV-2, PIV-3, and RSV on a NanoChip 400 electronic microarray. The ResPlex II assay (Genaco Biomedical Products, Inc., Huntsville, AL) detects InfA, InfB, PIV-1 to PIV-4, RSV, hMPV, rhinovirus, enterovirus, and the SARS coronavirus on a Luminex 100 instrument (Luminex, Austin, TX). Both assays exhibited specificities comparable to those of cell culture and the monoplex real-time reverse transcription (RT)-PCR. However, the sensitivities of both assays were lower than the sensitivity of the monoplex real-time RT-PCR. The multiplex ligation-dependent probe amplification (MLPA) technology (27) uses a simple-to-perform, multiplex PCR method which is able to amplify up to 45 different targets simultaneously. MLPA is based on the oligonucleotide ligation assay, and identification is accomplished by size by using gel electrophoresis methods. MLPA has three steps: first, an annealing step hybridizes the probes to their target regions; second, a ligation step links the two probes; and third, the final PCR exponentially amplifies the ligated probes with only two primers (Fig. 1). So far, MLPA has mainly been used to detect changes in the copy numbers of specific chromosomal regions (27), in expression profiling studies (6), for the detection of CpG methylation of genes (22), and for the detection of recombination events (16). We developed a multiparameter test (the RespiFinder assay) that is based on the MLPA technology and that can be used clinically to detect infectious disease agents. The RespiFinder assay allows the detection and differentiation of 15 respiratory viruses and one internal amplification control (IAC) (2, 14). The test includes 14 viruses involved in RTIs. These are InfA, influenza virus B (InfB), PIV-1 to PIV-4, respiratory syncytial virus A (RSVA), respiratory syncytial virus B (RSVB), rhinovirus, Cor-229E, Cor-OC43, CorNL63, hMPV, and adenovirus. Additionally, the test includes a probe for InfA H5N1. The RespiFinder assay was validated with 144 clinical samples, and the results were compared with those of cell culture and an RSV-specific immunochromatography assay (ICA). We demonstrate that the RespiFinder assay provides an excellent tool for the simultaneous detection of 15 respiratory viruses.

MATERIALS AND METHODS Viral cultures and monoplex real-time RT-PCR. Serial dilutions of cultures of RSVA, RSVB, InfA, InfB, rhinovirus, Cor-OC-43, Cor-229E, Cor-NL63, PIV-1, PIV-2, PIV-3, PIV-4, and hMPV and the results of the monoplex real-time

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FIG. 1. Overview of the RespiFinder technology. A one-step RTPCR is performed with specific primers for all targets (steps 1A and 1B). Subsequently, an MLPA reaction is performed with MLPA probes specific for all targets (steps 2, 3, and 4). An MLPA probe consists of two oligonucleotides: one synthetic oligonucleotide and one M13-derived oligonucleotide. The synthetic oligonucleotide contains a universal forward priming site, and the M13-derived oligonucleotide contains a universal reverse priming site. In addition, the M13-derived oligonucleotide contains a unique stuffer sequence. The length of this stuffer sequence is specific for each probe and varies between the different probes. The length of the MLPA probe is the combined length of both oligonucleotides. This length is unique for each probe due to the specific stuffer sequence. The two oligonucleotides hybridize specifically to the target adjacent to each other. Subsequently, the two oligonucleotides are joined by ligation. The ligated oligonucleotides are amplified by one universal primer set. After amplification, the MLPA reaction is analyzed by electrophoresis (step 5). Each MLPA probe can be discerned due to its specific length. Recently, the protocol has been further optimized by combining the probe ligation (step 3) and probe amplification (step 4) in one reaction.

RT-PCR obtained with the dilutions were kindly provided by H. G. Niesters, Department of Virology, Erasmus MC, Rotterdam, The Netherlands. Clinical samples. A total of 144 nasal wash specimens (from both adults and children) were submitted for the routine diagnosis of viral infection; of these, 110 samples were tested by cell culture on four different cell lines (Virology Department, University Hospital St. Radboud, Nijmegen. The Netherlands). This included adenovirus, hMPV, InfA, InfB, PIV-1 to PIV-4, rhinovirus, and RSV. The samples were not routinely checked for the presence of coronaviruses. A rapid ICA was performed for the detection of RSV in 34 samples from children by using the RSV Respi-Strip from Coris BioConcept (Gembloux, Belgium). All clinical samples were stored at ⫺80°C until further analysis by the RespiFinder assay. Nucleic acid extraction. Viral RNA or DNA was isolated by using the automated MagNA Pure LC system (Roche Diagnostics, Almere, The Netherlands). The MagNA Pure LC total nucleic acid isolation kit and the total nucleic acid lysis extraction MagNA Pure protocol were applied. Extraction was performed according to the manufacturer’s instructions. Briefly, 200 ␮l of starting material was used, and the purified nucleic acid was eluted in a final volume of 100 ␮l. Before the start of extraction, 5 ␮l of the IAC, which contained an encephalomyocarditis virus (EMC) RNA transcript, was added to the lysed samples. In vitro transcripts of viral targets. Synthetic viral target genes, which contained both the PCR primer regions and the MLPA probe sequence, were constructed by using the software package of DNA Works (version 3.1). The DNA Works software calculates the composition and the number of oligonucleotides required to synthesize the viral target. The oligonucleotides generated are characterized by highly homogeneous melting temperatures and a minimized tendency for hairpin formation. By using a two-step PCR protocol, the synthetic viral target gene can easily be synthesized and amplified (15).

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The amplification products were purified with an MSB Spin PCRapace kit (Invitek, Berlin, Germany) and were subsequently cloned in pGEM-T Easy vector system II (Promega, Leiden, The Netherlands). The nucleotide sequences of the cloned viral target genes were sequenced on an ABI 3100 DNA capillary sequencer. All cloned viral targets were linearized and transcribed in vitro from the SP6 promoter by using the Riboprobe in vitro transcription kit (Promega, Leiden, The Netherlands). Residual plasmid DNA was removed by DNase treatment (TURBO DNA-free; Ambion, Huntingdon, United Kingdom), according to the manufacturer’s instructions. The concentration of the SP6 RNA transcripts was determined by measuring the absorbance at 260 nM (1 unit of the optical density at 260 nm is equal to 40 ␮g/ml of RNA), and the absence of residual plasmid DNA was checked by performing a real-time PCR without an RT step. Aliquots of the RNA transcripts were stored at ⫺20°C, and dilutions were made in Tris-EDTA (pH 7.6) containing 1 ␮g/ml of carrier DNA (herring sperm DNA; Fermentas, St. Leon-Rot, Germany). IAC. The IAC was a SP6 RNA transcript of the polyproteon gene from EMC. The IAC was produced as described above. Twofold serial dilutions of the IAC were spiked into a clinical sample which previously tested virus negative by the RespiFinder assay. Subsequently, the spiked clinical samples were analyzed by the RespiFinder assay. The optimal spiked concentration was defined as two times the lowest detectable concentration. Preamplification. A one-step RT-PCR protocol was performed with a OneStep RT-PCR kit (Qiagen, Hilden, Germany). Combined RT and multiplex target amplification PCR were performed in a 25-␮l reaction mixture, according to the manufacturer’s instructions, in the presence of all preamplification primers (Table 1). The mixture contained 0.2 ␮M of each primer and 10 ␮l of the RNA or DNA sample. Amplification was performed on a T1 thermocycler (Biometra, Go ¨ttingen, Germany), as follows: an initial cycle of 30 min at 50°C and 15 min at 95°C, followed by 30 cycles of 30 s at 94°C, 30 s at 55°C, and 60 s at 72°C and, finally, a 10-min extended elongation. Primer and probe design. The primers and probes were designed against conserved genes within each virus. The sequences from these genes were obtained from GenBank and from the Los Alamos influenza virus database (http: //www.flu.lanl.gov/). The sequences were aligned by using the Clustal X program (version 1.81) to identify highly conserved regions within each gene. PCR primers and MLPA probes were designed on the basis of the sequences of these highly conserved regions. The primers were designed with Primer3 software (version 0.2) (http://primer3.sourceforge.net/). These primers were used for both specific RT and target amplification. The primers flanked the target region of the MLPA probe. The MLPA probes were designed as described earlier (27). Subsequently, all primers and probes were evaluated by performing a BLAST analysis against the sequences in the NCBI database. The primers and probes were approved when no mismatches within the critical regions of the probes (e.g., no mismatch within 5 nucleotides from the ligation site) and primers (e.g., no mismatch at the 3⬘ end of a primer) were found. The primers and the probes were synthesized by Biolegio (Malden, The Netherlands) and are shown in Tables 1 and 2. MLPA reaction. MLPA analysis was performed essentially as described earlier (27), with minor modifications. The preamplification reaction mixture was diluted five times with sterile water. Two microliters of the diluted preamplification mixture was mixed with 3 ␮l of sterile water, 1.5 ␮l probe mixture, and 1.5 ␮l MLPA buffer (1.5 M KCl, 300 mM Tris-HCl, pH 8.5, 1 mM EDTA); and denaturation was performed for 5 min at 98°C in a thermocycler. After denaturation, the mixture was incubated for 1 h at 60°C and was subsequently diluted to 40 ␮l with ligation buffer (2.6 mM MgCl2, 5 mM Tris-HCl, pH 8.5, 0.013% nonionic detergents, 0.2 mM NAD). Ligation was performed by adding 1 U of the heat-labile ligase 65 enzyme and incubating at 54°C for 15 min, followed by ligase inactivation at 98°C for 5 min. Subsequently, 4 ␮l ligation mixture was used in a 20-␮l reaction volume containing 50 mM Tris-HCl, pH 8.3, 50 mM KCl, 1.5 mM MgCl2, deoxynucleoside triphosphates (0.2 mM each; Fermentas), 1 U Taq polymerase, and 0.2 ␮M of the two PCR primers (forward primer, 5⬘-GGGTT CCCTAAGGGTTGGA-3⬘; reverse primer, 5⬘-GTGCCAGCAAGATCCAATC TAGA-3⬘). Amplification was performed on a Biometra T1 thermocycler, as follows: an initial cycle of 2 min at 95°C, followed by 33 cycles of 30 s at 94°C, 30 s at 60°C, and 1 min at 72°C and, finally, a 10-min extended elongation. All buffers and enzymes for MLPA were obtained from MRC-Holland (Amsterdam, The Netherlands). Analysis of PCR products. The amplified MLPA products can be analyzed on different detection platforms, e.g., by electrophoresis in 2.5% agarose gels, by use of the HT DNA 5000 SE55 kit on a LabChip 90 system (Caliper LifeSciences, Teralfene, Belgium), in 6.5% acrylamide slab gels in a 4300 DNA analyzer (LI-COR Biosciences, Lincoln, NE), by capillary electrophoresis on a MegaBACE DNA analysis system (GE Healthcare Europe GmbH, Diegem, Belgium),

J. CLIN. MICROBIOL. TABLE 1. Sequences of the preamplification primers Virus

Primer

Sequence (5⬘–3⬘)

InfA

Forward Reverse

CAAGACCAATCCTGTCACCTCT ATCGATGGCGCATGCAACTGGCAAG

InfB

Forward Reverse

ATGTCGCTGTTTGGAGACACAATTG GCATCTTTTGTTTTTTATCCATTC

InfA/H5N1

Forward Reverse

TGCATGGGTCTCATATACAACA TCCATAGCCTTAGCTGTAGTGC

RSVA

Forward Reverse

TCCCATAATATACAAGTATGATCTCAA AACCCAGTGAATTTATGATTAGCA

RSVB

Forward Reverse

TGTGGTATGCTATTAATCACTGAAGA GGAGCCACTTCTCCCATCTC

PIV-1

Forward Reverse

TTCTGGAGATGTCCCGTAGG TCCTGTTGTCGTTGATGTCATA

PIV-2

Forward Reverse

TGGGGATAATACAACAATCTGC AGAAAGCAAGTCTCAGTTCAGC

PIV-3

Forward Reverse

TCAATCTCAACAACAAGATTTAAGAA GACACCCAGTTGTGTTGCAG

PIV-4

Forward Reverse

TACAGGCCACATCAATGCAG GCATGTTCTGCATCTCTGGA

Rhinovirus

Forward Forward Reverse

GCCTGCGTGGCTGCC CCTGCGTGGCGGCC GAAACACGGACACCCAAAGTAGT

Cor-229E

Forward Reverse

CGCAGCCGGTGGAAAAGACAGCCTAA AGCATAGCAGCTGTAGACGGCAC AAGC

Cor-OC43

Forward Reverse

AAGAGCTCAACCCAAGCAAA ATACCATCGTGGCAGCAGTT

Cor-NL63

Forward Reverse

GGCTGCGTTACTTTGGCTTTAAAGAAC TTAGGTTTTG GACGCTCCAACGAGGTTTCTTCAACTG

hMPV

Forward Reverse

CAAAGAGGCAAGAAAAACAATGG GCCTGGCTCTTCTGACTGTGGTCTC

Adenovirus

Forward

GCCCATGCGCTGGACATGACTTTTGAG GTGGATCCCATGGA GACATGACTTTTGAGGTGGATCCCA TGGA TTATGTGGTGGCGTTGCCGGC AAGAAGCAAGAGGCTTCTTATGTGGTG GCGTTACCGGC

Forward Reverse Reverse

EMC (IAC)

Forward Reverse

ACATGTAACCGCCCCCATT TCCACGCACGCACTACTATG

and/or in an ABI 3100 genetic analyzer (Applied Biosystems, Nieuwerkerk a/d IJssel, The Netherlands). For detection on the 4300 DNA analyzer, an IR-700-labeled reverse primer was used in the final PCR. The final PCR mixture was diluted 30 times and was analyzed on the 4300 DNA analyzer according to the manufacturer’s instruction. When analysis was performed on a MegaBACE DNA analysis system or an ABI 3100 genetic analyzer, a 6-carboxyfluorescein-labeled forward primer was used in the final PCR. The final PCR mixture was diluted 10 times and was subsequently treated according to the manufacturers’ instructions. All clinical samples were analyzed by capillary electrophoresis on a MegaBACE DNA analysis system or an ABI 3100 genetic analyzer.

RESULTS MLPA reaction. The MLPA technology allows highly complex analyses of up to 45 targets in a single reaction. However, a standard MLPA reaction requires at least 6,000 copies of

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TABLE 2. Target genes and sequences of virus specific regions of the MLPA probes Virus

Gene

MLPA oligonucleotide

Sequence of virus-specific regions of MLPA probe (5⬘–3⬘)

InfA

Matrix protein gene (M1)

Synthetic Long

CCATGCACGCTCACCGTGCCCAGTGAGCGAGG ACTGCAGCGTAGACGCTTTGTCCAAAATGCCCTCAATG GGAATG

InfB

Matrix protein gene (M1)

Synthetic Long

GACAGAAGATGGAGAAGGCAAAGCAGA ACTAGCAGAAAAATTACACTGTTGGTTCGGTGGGAA AGAA

InfA H5N1

Matrix protein gene (M1)

Synthetic Long

CIGTIACTACIGAAGTGGCTTTTGGCCTA GTGTGTGCCACTTGTGAGCAGATTGCAGATTCACAGCA

RSVA

Major nucleocapsid protein gene (N)

Synthetic Long

GGCTCTTAGCAAAGTCAAGTTGAATGATACACTC AACAAAGATCAACTTCTGTCATCCAGCAAATACACCAT CCAACGGA

RSVB

Major nucleocapsid protein gene (N)

Synthetic Long

GTCCAGGTTAGGAAGGGAAGACACTATAAAGATACTT AAAGATGCTGGATATCATGTTAAAGCTAATGGAGTAG ATATAACAA

PIV-1

Hemagglutinn-neuraminidase gene (HN)

Synthetic Long

CAGGATGTGTTAGACTACCTTCATTATCAATTGGT GATGCAATATATGCGTATTCATCAAACTTAATCACTCA AGGATGTGC

PIV-2

Hemagglutinn-neuraminidase gene (HN)

Synthetic Long

CAGGACTATGAAAACCATTTACCTAAGTGATGG AATCAATCGCAAAAGCTGTTCAGTCACTGCTATACCAG GAGGTTGT

PIV-3

Hemagglutinn-neuraminidase gene (HN)

Synthetic Long

CCATCTGTTGGACCAGGGATATACTACAAA GGCAAAATAATATTTCTCGGGTATGGAGGTCTTGAACA TCCAA

PIV-4

Hemagglutinn-neuraminidase gene (HN)

Synthetic

GATTATACATTAACTATTAATCCAAGATCTGGCTGG GATG ACATCAAGATCAGAGCTTATAGAGCATTATCCAGAGAT TTGC

Long

Rhinovirus

5⬘ untranslated region polyprotein gene (PP)

Synthetic Long

GACAIGGTGTGAAGAGCCCCGTGTGCTIIIITTGAITC CTCC GGCCCCTGAATGTGGCTAACCTTAACCC

Cor-229E

Nucleocapsid protein gene (NP)

Synthetic Long

CCCAGAGACCTTGACCACAACTTTGGAAGT GCAGGTGTTGTGGCCAATGGTGTTAAAGCTAAAGGC TATC

Cor-OC43

Nucleocapsid protein gene (NP)

Synthetic Long

CTATTGCACCAGGAGTCCCAGCTACTGAA GCTAAGGGGTACTGGTACAGACACAACAGACGTTCTTT TAAAAC

Cor-NL63

Nucleocapsid protein gene (NP)

Synthetic Long

CCAGTCGAAGTCACCTAGTTCTTCTGGTA CTTCCACTCCTAAGAAACCTAATAAGCCTCTTTCTCAAC CCAGGGCT

hMPV

Nucleocapsid protein gene (NP)

Synthetic

GCTCATGCATCCCACAAAATCAGAGGCCTTCAGCA CCAG ACACACCAATAATTTTATTATGTGTAGGTGCCTTAATAT TCACTAAACTAGCATCAA

Long

Adenovirus

Hexon gene (H)

Synthetic Synthetic Long

EMC (IAC)

Polyprotein gene (PP)

Synthetic Long

target DNA (27). We made some modifications to the MLPA technology to obtain the sensitivity required for the effective detection of infectious pathogens. An RT step was introduced for the conversion of RNA into DNA. This was followed by a PCR to amplify the target DNA, which was then present at levels above the detection level of MLPA. Subsequently, an

GAAGTTTTCGACGTGGTCCGAGTGCACCAGCCGCA CCGC GAAGTTTTCGACGTGGTCAGTGTGCATCAGCCACA CCGC GGCGTCATCGAGGCCGTCTACCTGCGCACACCGTTCTC GCAGTCAGGTGAAGCACCCAGACTTGCCTCCTTGT GAGAGGCCGCACCTTGGTAGTAAATAGACACATGGCC GAGT

MLPA reaction was performed and comprised a probe hybridization step, a probe ligation step, and a probe amplification step. A schematic representation of the RespiFinder assay is shown in Fig. 1. An IAC is included in the assay to discriminate between samples with true-negative results and samples with false-neg-

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FIG. 3. Detection of the IAC in spiked serial virus dilutions on a 2.5% agarose gel. RespiFinder assay analysis was performed with fivefold serial dilutions of the supernatant of a PIV-1 culture. Lanes: 1, undiluted; 2, diluted 51; 3, diluted 52; 4, diluted 53; 5, diluted 54; 6, diluted 55; 7, diluted 56; 8, blank. Each dilution except the blank was spiked with the IAC.

FIG. 2. Overview of the RespiFinder probes and their length. nt, nucleotides.

ative results due to PCR failure. This added up to a total of 16 probes. The total lengths of the probes varied from 157 to 492 nucleotides. The sizes of the probes of the related viruses were clustered. Four clusters are distinguished: an influenza virus cluster of about 400 nucleotides, a PIV cluster of about 300 nucleotides, an RSV cluster of about 250 nucleotides, and a coronavirus cluster of about 170 nucleotides. An overview of all probes is presented in Fig. 2. MLPA probes. An MLPA probe consists of one short synthetic oligonucleotide and one phage M13-derived, long oligonucleotide probe (27). Each oligonucleotide contains a targetspecific hybridizing part and one universal priming site. In addition, the long oligonucleotide probe contains a stuffer sequence to facilitate size-based separation. The most conserved region within each viral family was selected to design the two hybridizing parts of the MLPA probe. The adenovirus group is a very large and heterogeneous group, including 51 different serotypes divided into six subgenera. To cover all six subgenera with one MLPA probe, we combined one long oligonucleotide probe with two synthetic oligonucleotides. This MLPA probe was tested with 15 different adenovirus serotypes covering the six subgenera. Included were serotypes 2, 4, 5, and 7, which are generally more often associated with RTIs (25), and serotypes 8, 9, 12, 19, 30, 31, 35, 37, 40, 48, and 49. All 15 serotypes could be detected by use of this probe (data not shown). Specificity. To asses the specificity of the primers and the probes, all PCR primers and MLPA probes were tested in either a monoplex or a multiplex MLPA reaction with different samples. No cross-reactivity among the 15 viral probes and the IAC probe was observed when they were tested with culture samples of individual viruses. In addition, clinical samples which tested positive for other pathogens by routine diagnostic analysis by pathogen-specific PCR assays were analyzed by the RespiFinder assay. These samples contained enterovirus, echovirus, coxsackievirus, and herpes simplex virus type 1, as well as the bacterial pathogens Mycoplasma pneumoniae, Chlamydia

pneumoniae, Legionella pneumophila, Bordetella pertussis, Staphylococcus warneri, Staphylococcus intermedius, Staphylococcus haemolyticus, Staphylococcus epidermidis, Enterococcus faecalis, Pseudomonas spp., Haemophilus influenzae, Haemophilus parainfluenzae, and Streptococcus spp. No sample showed any crossreactivity with the RespiFinder assay probes (data not shown). Internal control. The use of an IAC allows discrimination between a true-negative result and a false-negative result due to a PCR/MLPA failure. However, since the MLPA reaction uses only two primers in the final PCR, the amplification of any respiratory virus-specific MLPA probe competes with the amplification of the IAC MLPA probe. Figure 3 shows the results of the RespiFinder assay with fivefold serial dilutions of a PIV-1 culture, all of which were spiked with an equal amount of IAC. Only a weak IAC signal was detected in the presence of the highest PIV-1 concentration. As the PIV-1 concentration decreased, the IAC signal increased. This demonstrates competition between simultaneously amplified MLPA probes. Analytical sensitivity: RNA transcripts and serial virus dilutions. First, to determine the analytical sensitivity of the RespiFinder assay, serial dilutions of viral RNA transcripts of all RNA viruses and serial dilutions of a plasmid with the adenovirus target sequence were analyzed by the RespiFinder assay, and the reactions were analyzed on a LI-COR 4300 DNA analyzer. The limit of detection of the 15 viral RNA transcripts did not vary significantly, and for each viral probe an analytical detection limit of 10 to 20 copies was determined. Second, the sensitivity of the RespiFinder assay was compared to that of the monoplex real-time PCR. Nucleic acid preparations from fivefold serial dilutions of culture supernatants of 13 viruses (no InfA H5N1 or adenovirus cultures were available) were tested. The results are shown in Table 3. In the monoplex real-time PCR, 20 ␮l of an RNA or a DNA sample was used, whereas 10 ␮l of an RNA or a DNA sample was used in the preamplification step of the RespiFinder assay. The results indicate that the sensitivity of the RespiFinder assay was comparable to that of the monoplex real-time RT-PCR. Validation with respiratory specimens. To validate the performance of the RespiFinder assay with clinical samples, 110 nasal lavage fluid specimens from patients with symptoms of RTIs were analyzed retrospectively. All clinical samples were analyzed by capillary electrophoresis on a MegaBACE DNA

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TABLE 3. Sensitivity of RespiFinder assay compared to that of monoplex real-time RT-PCRa Highest viral dilution detected by: Virus

RespiFinder assay

Real-time RT-PCR

RSVA RSVB InfA InfB Rhino Cor-OC43 Cor-229E Cor-NL63 PIV-1 PIV-2 PIV-3 PIV-4 hMPV

4 5 6 7 7 6 5 6 6 7 6 6 5

4 5 6 7 7 5 6 6 7 7 6 7 4

a

Fivefold serial dilutions of all indicated viruses were analyzed.

analysis system or an ABI 3100 genetic analyzer. Typical results of this RespiFinder assay screening and analyses by capillary electrophoresis are shown in Fig. 4. The results of the validation assay are shown in Tables 4 and 5. The RespiFinder assay identified the same virus as that identified by cell culture in 37 of 39 samples (94.9%). The two aberrant results were for samples in which an untypeable influenza virus was detected by cell culture and an InfA was detected by RespiFinder assay and a sample in which PIV-3 was detected by cell culture and hMPV was detected by the RespiFinder assay. The eight adenovirus infections detected were caused by adenovirus type 2 (subgenera C) and adenovirus types 3 and 7 (subgenera B). By cell culture, 71 clinical samples were found to be negative. In 22 (31%) of these culture-negative samples, a virus was identified by the RespiFinder assay. These included nine rhinovirus infections, five RSVA infections, one RSVB infection, two hMPV infections, two InfA infections, one PIV-3 infection, one adenovirus infection, and a rhinovirus and PIV-1 coinfection. In addition, one Cor-NL63 infection and two Cor-OC43 infections were detected by the RespiFinder assay. The coro-

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TABLE 4. Analysis of concordant results between RespiFinder assay and cell culture for 110 clinical samplesa Cell culture and RespiFinder assay result

No. (%) of samples

Adenovirus hMPV InfA PIV-1 PIV-3

8 2 4 1 4

Rhinovirus

5

RSV

13

Negative Total

45 82 (74.5)

Remarks

Including serotypes 2, 3, and 7

1 CIb with rhinovirus detected by RespiFinder assay 1 CI with hMPV detected by RespiFinder assay 7 RSVA (1 CI with adenovirus), 5 RSVB, and 1 CI of RSVA ⫹ RSVB detected by RespiFinder assay

a The results were considered consistent if the virus identified by cell culture was the same virus as that identified by the RespiFinder assay. Additional viruses identified by the RespiFinder assay are indicated. An RSV-positive result by cell culture was considered consistent with the RespiFinder assay result if either RSVA or RSVB was identified by the RespiFinder assay. b CI, coinfection.

naviruses were not included in the cell culture screening. Therefore, the coronavirus results of the RespiFinder assay are reported but were not used in the validation of RespiFinder assay. In total, five coinfections were detected by RespiFinder assay. These involved three coinfections of rhinovirus with PIV-1, PIV-3, and hMPV, respectively, and two coinfections of RSVA with adenovirus and RSVB, respectively. No coinfection was detected by cell culture. Overall, the RespiFinder assay detected 66 (60%) viruses in the 110 samples. All viruses involved in the coinfections were counted individually, and the three coronavirus infections were not included. Cell culture detected 39 (35.5%) viruses. This is an increase in diagnostic yield of 24.5%. With two samples, no signal was observed by

FIG. 4. Results of the RespiFinder assay with two clinical samples which were analyzed by capillary electrophoresis. Sample 1 represents a clinical sample with a rhinovirus (Rhino) infection. The electropherogram shows a signal at the position of the rhinovirus probe and the IAC. Sample 2 represents a clinical sample with no viral infection. Only the IAC signal was detected in the electropherograms. Contr, internal amplification control.

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TABLE 5. Analysis of nonconsistent results between RespiFinder assay and cell culturea Cell culture result (no. of samples)

RespiFinder assay result

No. (%) of samples

Untypeable inflenza virus (1)

InfA

1

PIV-3 (1)

hMPV

1

Negative (26)

Rhinovirus Cor-NL63 Cor-OC43 RSVA RSVB hMPV InfA Adenovirus PIV-3 Rhinovirus ⫹ PIV-1 Failureb

9 1 2 5 1 2 2 1 1 1

Total

TABLE 6. Comparison of RespiFinder assay and RSV-specific ICA results for 34 clinical samples RSV-specific ICA score (no. of samples)

RSV score

Positive (15)

Positive (12)

RSVA (6) RSVB (5) RSVB ⫹ rhinovirus (1)

Negative (2)

InfA (1) Negative (1)

Negative (19)

28 (25.5)

the RespiFinder assay in the initial screening. Upon retesting, one sample again failed to show any signal. In addition, 34 clinical samples which were routinely tested by the RSV-specific ICA were retrospectively analyzed by the RespiFinder assay (Table 6). Among the 15 samples RSV positive by the RSV-specific ICA, 12 samples were also RSV positive by the RespiFinder assay. The RespiFinder assay detected InfA in a sample which scored weakly positive by the RSV-specific ICA. The other two samples positive by the RSVspecific ICA were negative and failed to amplify the internal control in the RespiFinder assay. Retesting of the last sample again showed no amplification of the internal control. Three (15.8%) of the 19 samples which tested negative by ICA were also negative by the RespiFinder assay. In six (31.6%) samples, an RSV infection was detected by the RespiFinder assay, and these comprised four RSVA infections and two RSVB infections. In the remaining 10 (52.6%) samples, additional virus infections were detected by the RespiFinder assay. These included four InfA infections, four rhinovirus infections, one Cor-OC43 infection, and a Cor-OC43 and Cor-NL63 coinfection. The sensitivity and specificity of the RespiFinder assay were assessed in relation to the results of cell culture and ICA (Table 7). In agreement with the cell culture results, the RespiFinder assay identified 10 samples with adenovirus infections (9.1%), 6 with hMPV infections (5.5%), 7 with InfA infections (6.4%), 2 with PIV-1 infections (1.8%), 5 with PIV-3 infections (4.5%), 16 with rhinovirus infections (14.5%), and 19 with RSV infections (17.3%). In addition, the RespiFinder assay detected 27 additional positive samples, including 2 positive for adenovirus, 4 for hMPV, 2 for InfA, 1 for PIV-1, 1 for PIV-3, 11 for rhinovirus, and 6 for RSV. One sample with a false-negative result for PIV-3 was observed by the RespiFinder assay. Compared with the results of ICA, the RespiFinder assay detected 18 samples positive for RSV (52.9%), corresponding to a specificity of 82.4% and a sensitivity of

Additional virus(es) detected

Failurea (1)

a

The results were considered nonconsistent if the virus identified by cell culture was not identified by the RespiFinder assay. b No IAC signal.

RespiFinder assay result (no. of samples)

a

Negative (13)

Negative (3) InfA (4) Rhinovirus (4) Cor-OC43 (1) Cor-OC43 ⫹ Cor-NL63 (1)

Positive (6)

RSVA (4) RSVB (2)

No IAC signal.

80%. Six additional RSV-positive samples were observed by the RespiFinder assay. The results for three samples which scored RSV positive by ICA were not confirmed by the RespiFinder assay. DISCUSSION The number of possible viral agents involved in RTIs is high, and new viruses are still emerging. In recent years, five new viruses, including human bocavirus (1), the SARS coronavirus (4), hMPV (31), and coronaviruses NL63 (32) and HKU1 (36), were identified to play a role in RTIs. Although the gold standard for the laboratory detection of respiratory viruses is viral culture, monitoring of this increasing number of respiratory viruses solely by viral culture is not possible for practical reasons. PCR is a fast and sensitive alternative. However, the use of conventional PCR techniques is not practical in a study for the detection of a broad spectrum of pathogens due to the handling time and the high reagent costs (19). Here we present a new multiparameter test that is based on the MLPA technology and that is able to detect 15 respiratory viruses simultaneously. In order to obtain the required sensitivity, the MLPA technology was adapted by incorporating a preamplification step. This preamplification step involves an RT step and a 30-cycle target amplification step. Due to the introduction of the preamplification step, the hybridization time in the MLPA reaction could be reduced to 1 h, while the original MLPA protocol required a hybridization time of 16 h. As a result, the whole RespiFinder assay could be completed within a working day. In the initial experiments, the RespiFinder assay products were analyzed on 2.5% agarose gels. However, due to the complexity of the RespiFinder assay, the resolution of the agarose gel was insufficient to distinguish all products amplified by MLPA. The RespiFinder assay reactions were also analyzed on a LabChip 90 system from Caliper LifeSciences. The resolution of this system was also not sufficient for the

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TABLE 7. Sensitivity and specificity of RespiFinder assay compared with those of cell culture and an RSV-specific ICAa No. of samples with the following CC or CC/ICA result and RF resultb: Virus

CC⫹ or CC⫹/ICA⫹ and RF⫹

CC⫺ or CC⫺/ICA⫺ and RF⫹

CC⫹ or CC⫹/ICA⫹ and RF⫺

CC⫺ or CC⫺/ICA⫺ and RF⫺

Specificity (%)

Sensitivity (%)

Adenovirus hMPV InfA PIV-1 PIV-3 Rhinovirus RSV

8 2 5 1 4 5 13/12

2 4 2 1 1 11 6/6

0 0 0 0 1 0 0/2

101 105 104 109 105 95 92/13

98.2 96.4 98.2 99.1 99.1 90.1 94.6/81.8c

100 100 100 100 80 100 100/85.7c

a b c

The RespiFinder assay results for coronaviruses were not validated. CC, cell culture; RF, RespiFinder assay; ⫹, positive result; ⫺, negative result. Data represent the results by cell culture/ICA.

nonambiguous identification of all individual products amplified by MLPA. However, due to the clustering of probes of more related viruses, use of the LabChip 90 system allowed the detection of the individual probes for rhinovirus, adenovirus, and hMPV and the four probe clusters for influenza virus, PIV, RSV, and coronavirus. On high-resolution electrophoresis systems, such as the LI-COR 4300 DNA analyzer, the MegaBACE DNA analysis system, and the ABI 3100 genetic analyzer, all individual probes could be clearly distinguished. Well-designed MLPA probes have the ability to discriminate between single-nucleotide polymorphisms (27). The viral MLPA probes require a more generic design, as viruses, especially RNA viruses, show a great deal of genetic variability. Therefore, a major concern in the design of the MLPA probes was the compatibility of virus-specific probes with as many known viral sequences as possible, including those of the serotypes common among humans. However, this generic design should not compromise the specificity of the probe. The probes were positioned in well-conserved regions. No mismatch within 5 nucleotides from the ligation site was tolerated. With the adenovirus-specific probe two short synthetic oligonucleotides were combined with one M13-derived long oligonucleotide probe to enclose all 51 serotypes of the heterogeneous adenovirus group. No cross-reactivity was detected with any of the probes. The sensitivity and the specificity of the RespiFinder assay were assessed by comparison of the results of the RespiFinder assay to those of cell culture obtained with 110 clinical samples. All samples were spiked with the IAC. The spiking was done after addition of the lysis buffer in order to prevent degradation of the IAC. For one (1%) sample, the RespiFinder assay failed to produce a result. The RespiFinder assay detected 27 (24.5%) viruses which were missed by cell culture. These included 2 adenoviruses, 4 hMPVs, 2 InfAs, 1 PIV-1, 1 PIV-3, 11 rhinoviruses, and 6 RSVs. This increase in diagnostic yield is in accordance with the findings of other studies that used molecular methods (10, 23). One sample with a false-negative result for PIV-3 was observed by the RespiFinder assay. Among the eight adenoviruses detected, three were of different serotypes (serotypes 2, 3, and 7) representing two different subgenera (subgenera B and C). This illustrates the ability of the generic adenovirus probe to detect different serotypes in clinical samples. The RespiFinder assay found an incidence of coinfection of 7.8%, whereas cell culture did not detect any double infec-

tions. The percentage of mixed infections that we detected is in agreement with the percentages detected in other studies, which showed incidences of coinfections of 3.4% (34), 6.1% (21), and 18.6% (3). Compared to the results of a commercial ICA-based rapid assay for RSV with 34 clinical samples, the RespiFinder assay detected 18 (52.9%) RSV infections, corresponding to a specificity of 82.4% and a sensitivity of 80%. The results for two RSV-positive samples were not confirmed. This included one sample which scored weakly positive by the rapid assay for RSV. The RespiFinder assay detected an InfA infection in this sample. In addition, the RespiFinder assay detected six additional RSV-positive samples. Additional viruses were detected in 52.6% of the ICA RSV-negative samples, including InfA, rhinovirus, Cor-OC43, and Cor-NL63. In conclusion, we have developed a new multiparameter respiratory assay based on the MLPA technique for the detection of 15 respiratory viruses plus an ICA. The analytical sensitivity of the RespiFinder assay matches the sensitivity of the monoplex real-time RT-PCR. The validation with clinical samples shows that the RespiFinder assay gives an excellent overall performance. The assay does not need specialized equipment but makes use of the PCR and capillary electrophoresis systems generally available in molecular laboratories. The assay can be performed within one working day and is suitable for implementation in a diagnostic setting. Implementation of this assay for routine diagnostics allows the fast analysis of samples for a broad spectrum of pathogens at a reduced cost compared to the costs of individual monoplex real-time RT-PCR assays. At present, the full analytical power of the RespiFinder assay can be used only when the results are analyzed on a high-resolution system like a capillary electrophoresis system. However, by adapting the design of the MLPA probes, it will also be possible to identify most probes on LabChip systems, like the Caliper LabChip 90 system, the Experion system (BioRad Laboratories, Hercules, CA), or the 2100 bioanalyzer (Agilent Technologies, Foster City, CA). The MLPA technology allows the highly complex analysis of up to 45 fragments. This gives room for future expansion of the number of probes in the RespiFinder assay. Recently, four bacterial probes, including probes for Mycoplasma pneumoniae, Chlamydophila pneumoniae, Legionella pneumophila, and Bordetella pertussis, have been added to the RespiFinder assay. This allows the detection in a clinical sample of 19 pathogens and one IAC in

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one reaction. In addition, for better implementation in a diagnostic setting, the RespiFinder assay protocol was recently adapted by combining the probe ligation step and the probe amplification step in a single reaction. As a result, the RespiFinder assay protocol consists at present of four steps, i.e., preamplification (one-step RT-PCR), probe hybridization, probe ligation/amplification, and probe detection. ACKNOWLEDGMENTS We thank Bert Niesters (Erasmus Medical Centre, Rotterdam) for the serial dilutions of viral RNA and performing the monoplex realtime PCR analysis. We thank Eric Claas (Leiden University Medical Centre) for providing us with the DNA of the different adenovirus serotypes. Sandra Bokkers (Canisius Wilhelmina Hospital Nijmegen) is acknowledged for technical assistance. In addition, we thank Lothar Kruska and Andre´ Frontzek (Stein ⫹ Kollegen, Mo ¨nchengladbach, Germany) for assisting us with the cross-reactivity testing. The research described here has been facilitated by a grant provided by the Dutch Ministry of Economic Affairs (grant TSGE3074). REFERENCES 1. Allander, T., M. T. Tammi, M. Eriksson, A. Bjerkner, A. Tiveljung-Lindell, and B. Andersson. 2005. Cloning of a human parvovirus by molecular screening of respiratory tract samples. Proc. Natl. Acad. Sci. USA 102:12891–12896. 2. Beld, M., R. Minnaar, J. Weel, C. Sol, M. Damen, H. van der Avoort, P. Wertheim-van Dillen, A. van Breda, and R. Boom. 2004. Highly sensitive assay for detection of enterovirus in clinical specimens by reverse transcription-PCR with an armored RNA internal control. J. Clin. Microbiol. 42:3059–3064. 3. Coiras, M. T., J. C. Aguilar, M. L. Garcia, I. Casas, and P. Perez-Brena. 2004. Simultaneous detection of fourteen respiratory viruses in clinical specimens by two multiplex reverse transcription nested-PCR assays. J. Med. Virol. 72:484–495. 4. Drosten, C., S. Gunther, W. Preiser, S. van der Werf, H. R. Brodt, S. Becker, H. Rabenau, M. Panning, L. Kolesnikova, R. A. Fouchier, A. Berger, A. M. Burguiere, J. Cinatl, M. Eickmann, N. Escriou, K. Grywna, S. Kramme, J. C. Manuguerra, S. Muller, V. Rickerts, M. Sturmer, S. Vieth, H. D. Klenk, A. D. Osterhaus, H. Schmitz, and H. W. Doerr. 2003. Identification of a novel coronavirus in patients with severe acute respiratory syndrome. N. Engl. J. Med. 348:1967–1976. 5. Effler, P. V., M. C. Ieong, T. Tom, and M. Nakata. 2002. Enhancing public health surveillance for influenza virus by incorporating newly available rapid diagnostic tests. Emerg. Infect. Dis. 8:23–28. 6. Eldering, E., C. A. Spek, H. L. Aberson, A. Grummels, I. A. Derks, A. F. de Vos, C. J. McElgunn, and J. P. Schouten. 2003. Expression profiling via novel multiplex assay allows rapid assessment of gene regulation in defined signalling pathways. Nucleic Acids Res. 31:e153. 7. Erdman, D. D., G. A. Weinberg, K. M. Edwards, F. J. Walker, B. C. Anderson, J. Winter, M. Gonzalez, and L. J. Anderson. 2003. GeneScan reverse transcription-PCR assay for detection of six common respiratory viruses in young children hospitalized with acute respiratory illness. J. Clin. Microbiol. 41:4298–4303. 8. Falsey, A. R., E. E. Walsh, and F. G. Hayden. 2002. Rhinovirus and coronavirus infection-associated hospitalizations among older adults. J. Infect. Dis. 185:1338–1341. 9. File, T. M. 2003. Community-acquired pneumonia. Lancet 362:1991–2001. 10. Freymuth, F., A. Vabret, D. Cuvillon-Nimal, S. Simon, J. Dina, L. Legrand, S. Gouarin, J. Petitjean, P. Eckart, and J. Brouard. 2006. Comparison of multiplex PCR assays and conventional techniques for the diagnostic of respiratory virus infections in children admitted to hospital with an acute respiratory illness. J. Med. Virol. 78:1498–1504. 11. Greenberg, S. B. 2002. Respiratory viral infections in adults. Curr. Opin. Pulm. Med. 8:201–208. 12. Grondahl, B., W. Puppe, A. Hoppe, I. Kuhne, J. A. Weigl, and H. J. Schmitt. 1999. Rapid identification of nine microorganisms causing acute respiratory tract infections by single-tube multiplex reverse transcription-PCR: feasibility study. J. Clin. Microbiol. 37:1–7. 13. Gunson, R. N., T. C. Collins, and W. F. Carman. 2005. Real-time RT-PCR detection of 12 respiratory viral infections in four triplex reactions. J. Clin. Virol. 33:341–344. 14. Hoorfar, J., B. Malorny, A. Abdulmawjood, N. Cook, M. Wagner, and P. Fach. 2004. Practical considerations in design of internal amplification controls for diagnostic PCR assays. J. Clin. Microbiol. 42:1863–1868. 15. Hoover, D. M., and J. Lubkowski. 2002. DNAWorks: an automated method for designing oligonucleotides for PCR-based gene synthesis. Nucleic Acids Res. 30:e43.

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